Your search keyword '"Oesterhelt, D."' showing total 32 results

1. Multimeric options for the auto-activation of the Saccharomyces cerevisiae FAS type I megasynthase.

Author

Johansson P, Mulinacci B, Koestler C, Vollrath R, Oesterhelt D, and Grininger M

Subjects

Acyl Carrier Protein chemistry, Acyl Carrier Protein genetics, Acyl Carrier Protein metabolism, Amino Acid Sequence, Bacterial Proteins chemistry, Bacterial Proteins genetics, Bacterial Proteins metabolism, Catalysis, Catalytic Domain, Coenzyme A chemistry, Coenzyme A metabolism, Enzyme Activation, Fatty Acid Synthases genetics, Fatty Acid Synthases metabolism, Fatty Acids chemistry, Fatty Acids metabolism, Magnesium chemistry, Magnesium metabolism, Models, Chemical, Models, Molecular, Molecular Sequence Data, Molecular Structure, Mutation, Protein Binding, Protein Processing, Post-Translational, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins metabolism, Sequence Homology, Amino Acid, Transferases (Other Substituted Phosphate Groups) chemistry, Transferases (Other Substituted Phosphate Groups) genetics, Transferases (Other Substituted Phosphate Groups) metabolism, Fatty Acid Synthases chemistry, Protein Multimerization, Protein Structure, Tertiary, Saccharomyces cerevisiae Proteins chemistry

Abstract

The fungal type I fatty acid synthase (FAS) is a 2.6 MDa multienzyme complex, catalyzing all necessary steps for the synthesis of long acyl chains. To be catalytically competent, the FAS must be activated by a posttranslational modification of the central acyl carrier domain (ACP) by an intrinsic phosphopantetheine transferase (PPT). However, recent X-ray structures of the fungal FAS revealed a barrel-shaped architecture, with PPT located at the outside of the barrel wall, spatially separated from the ACP caged in the inner volume. This separation indicated that the activation has to proceed before the assembly to the mature complex, in a conformation where the ACP and PPT domains can meet. To gain insight into the auto-activation reaction and also into the fungal FAS assembly pathway, we structurally and functionally characterized the Saccharomyces cerevisiae FAS type I PPT as part of the multienzyme protein and as an isolated domain.

Published

2009

2. Influence of the charge at D85 on the initial steps in the photocycle of bacteriorhodopsin.

Author

Sobotta C, Braun M, Tittor J, Oesterhelt D, and Zinth W

Subjects

Amino Acid Sequence, Archaeal Proteins chemistry, Bacteriorhodopsins genetics, Hydrogen-Ion Concentration, Kinetics, Models, Molecular, Point Mutation, Potassium Chloride chemistry, Protein Isoforms chemistry, Sodium Chloride chemistry, Spectrum Analysis, Static Electricity, Bacteriorhodopsins chemistry, Halobacterium salinarum chemistry, Halorhodopsins chemistry

Abstract

Studies have shown that trans-cis isomerization of retinal is the primary photoreaction in the photocycle of the light-driven proton pump bacteriorhodopsin (BR) from Halobacterium salinarum, as well as in the photocycle of the chloride pump halorhodopsin (HR). The transmembrane proteins HR and BR show extensive structural similarities, but differ in the electrostatic surroundings of the retinal chromophore near the protonated Schiff base. Point mutation of BR of the negatively charged aspartate D85 to a threonine T (D85T) in combination with variation of the pH value and anion concentration is used to study the ultrafast photoisomerization of BR and HR for well-defined electrostatic surroundings of the retinal chromophore. Variations of the pH value and salt concentration allow a switch in the isomerization dynamics of the BR mutant D85T between BR-like and HR-like behaviors. At low salt concentrations or a high pH value (pH 8), the mutant D85T shows a biexponential initial reaction similar to that of HR. The combination of high salt concentration and a low pH value (pH 6) leads to a subpopulation of 25% of the mutant D85T whose stationary and dynamic absorption properties are similar to those of native BR. In this sample, the combination of low pH and high salt concentration reestablishes the electrostatic surroundings originally present in native BR, but only a minor fraction of the D85T molecules have the charge located exactly at the position required for the BR-like fast isomerization reaction. The results suggest that the electrostatics in the native BR protein is optimized by evolution. The accurate location of the fixed charge at the aspartate D85 near the Schiff base in BR is essential for the high efficiency of the primary reaction.

Published

2009

3. Hydration dependence of active core fluctuations in bacteriorhodopsin.

Author

Wood K, Lehnert U, Kessler B, Zaccai G, and Oesterhelt D

Subjects

Computer Simulation, Deuterium Exchange Measurement, Motion, Neutron Diffraction, Porosity, Protein Conformation, Bacteriorhodopsins chemistry, Bacteriorhodopsins ultrastructure, Models, Chemical, Models, Molecular, Purple Membrane chemistry, Purple Membrane ultrastructure, Water chemistry

Abstract

We used neutron scattering and specific hydrogen-deuterium labeling to investigate the thermal dynamics of isotope-labeled amino acids and retinal, predominantly in the active core and extracellular moiety of bacteriorhodopsin (BR) in the purple membrane and the dynamical response to hydration. Measurements on two neutron spectrometers allowed two populations of motions to be characterized. The lower amplitude motions were found to be the same for both the labeled amino acids and retinal of BR and the global membrane. The larger amplitude dynamics of the labeled part, however, were found to be more resilient than the average membrane, suggesting their functional importance. The response to hydration was characterized, showing that the labeled part of BR is not shielded from hydration effects. The results suggest that the inhibition of high-amplitude motions by lowering hydration may play a key role in the slowing down of the photocycle and the proton pumping activity of BR.

Published

2008

4. A quantitative model of the switch cycle of an archaeal flagellar motor and its sensory control.

Author

Nutsch T, Oesterhelt D, Gilles ED, and Marwan W

Subjects

Computer Simulation, Feedback physiology, Motion, Sensation physiology, Archaeal Proteins metabolism, Chemotaxis physiology, Flagella physiology, Halobacterium physiology, Mechanotransduction, Cellular physiology, Models, Biological, Molecular Motor Proteins physiology

Abstract

By reverse-engineering we have detected eight kinetic phases of the symmetric switch cycle of the Halobacterium salinarum flagellar motor assembly and identified those steps in the switch cycle that are controlled by sensory rhodopsins during phototaxis. Upon switching the rotational sense, the flagellar motor assembly passes through a stop state from which all subunits synchronously resume rotation in the reverse direction. The assembly then synchronously proceeds through three subsequent functional states of the switch: Refractory, Competent, and Active, from which the rotational sense is switched again. Sensory control of the symmetric switch cycle occurs at two steps in each rotational sense by inversely regulating the probabilities for a change from the Refractory to the Competent and from Competent to the Active rotational mode. We provide a mathematical model for flagellar motor switching and its sensory control, which is able to explain all tested experimental results on spontaneous and light-controlled motor switching, and give a mechanistic explanation based on synchronous conformational transitions of the subunits of the switch complex after reversible dissociation and binding of a response regulator (CheYP). We conclude that the kinetic mechanism of flagellar motor switching and its sensory control is fundamentally different in the archaeon H. salinarum and the bacterium Escherichia coli.

Published

2005

5. Probing origins of molecular interactions stabilizing the membrane proteins halorhodopsin and bacteriorhodopsin.

Author

Cisneros DA, Oesterhelt D, and Müller DJ

Subjects

Amino Acid Sequence, Crystallization, Halobacterium salinarum metabolism, Microscopy, Atomic Force, Molecular Sequence Data, Protein Folding, Protein Structure, Secondary, Protein Structure, Tertiary, Bacteriorhodopsins chemistry, Halorhodopsins chemistry

Abstract

Single-molecule atomic force microscopy and spectroscopy were applied to detect molecular interactions stabilizing the structure of halorhodopsin (HR), a light-driven chloride pump from Halobacterium salinarum. Because of the high structural and sequence similarities between HR and bacteriorhodopsin, we compared their unfolding pathways and polypeptide regions that established structurally stable segments against unfolding. Unfolding pathways and structural segments stabilizing the proteins both exhibited a remarkably high similarity. This suggests that different amino acid compositions can establish structurally indistinguishable energetic barriers. These stabilizing domains rather result from comprehensive interactions of all amino acids within a structural region than from specific interactions. However, one additional unfolding barrier located within a short segment of helix E was detected for HR. This barrier correlated with a Pi-bulk interaction, which locally disrupts helix E and divides a structural stabilizing segment.

Published

2005

6. Ultrafast conformational dynamics in cyclic azobenzene peptides of increased flexibility.

Author

Wachtveitl J, Spörlein S, Satzger H, Fonrobert B, Renner C, Behrendt R, Oesterhelt D, Moroder L, and Zinth W

Subjects

Amino Acid Sequence, Isomerism, Molecular Conformation, Molecular Sequence Data, Pliability, Spectrum Analysis, Azo Compounds chemistry, Models, Molecular, Peptides, Cyclic chemistry

Abstract

Structural changes of peptides containing the azobenzene dye 4-aminomethyl-phenylazobenzoic acid (AMPB) are studied with ultrafast spectroscopy. AMPB peptides are a new class of molecules where the photoisomerizable dye azobenzene is linked to the peptide moiety via a flexible methylene spacer. The ultrafast reactions in the femtosecond to nanosecond time domain are investigated for the optical switch AMPB, a linear and cyclic octapeptide, and a bicyclic octapeptide containing an additional disulfide bridge. These molecules with increasing conformational constraints are studied for the cis to trans and the trans to cis photoreactions. For the cis to trans reaction the isomerization of the chromophore occurs fast in the 1-ps range, whereas it is slower (10-ps range) in the trans to cis reaction. In all peptides the structural changes of the chromophore lead to modifications in the peptide structure in the 10-ps-1-ns time range. The results indicate that the chromophore AMPB acts simultaneously as a fast molecular switch and as a sensor for initial conformational dynamics in the peptide. Experiments in the mid-infrared range where the structural changes of the peptide backbone are directly observed demonstrate that the essential part of the structural dynamics in the bicyclic AMPB peptide occurs faster than 10 ns.

Published

2004

7. Crystal structure of halophilic dodecin: a novel, dodecameric flavin binding protein from Halobacterium salinarum.

Author

Bieger B, Essen LO, and Oesterhelt D

Subjects

Amino Acid Sequence, Archaeal Proteins genetics, Archaeal Proteins metabolism, Bacterial Proteins chemistry, Bacterial Proteins genetics, Crystallography, X-Ray, Dimerization, Genomics, Halobacterium salinarum metabolism, Models, Molecular, Molecular Sequence Data, Molecular Structure, Protein Structure, Tertiary, Protein Subunits chemistry, Protein Subunits metabolism, Sequence Alignment, Archaeal Proteins chemistry, Flavins metabolism, Halobacterium salinarum chemistry, Protein Structure, Quaternary

Abstract

A novel, 68 amino acid long flavoprotein called dodecin has been discovered in the proteome of Halobacterium salinarum by inverse structural genomics. The 1.7 A crystal structure of this protein shows a dodecameric, hollow sphere-like arrangement of the protein subunits. Unlike other known flavoproteins, which bind only monomeric flavin cofactors, the structure of the dodecin oligomer comprises six riboflavin dimers. The dimerization of these riboflavins along the re-faces is mediated by aromatic, antiparallel pi staggering of their isoalloxazine moieties. A unique aromatic tetrade is formed by further sandwiching of the riboflavin dimers between the indole groups of two symmetry-related Trp36s. So far, the dodecins represent the smallest known flavoproteins. Based on the structure and the wide spread occurrences in pathogenic and soil eubacteria, a function in flavin storage or protection against radical or oxygenic stress is suggested for the dodecins.

Published

2003

8. Subsecond proton-hole propagation in bacteriorhodopsin.

Author

Schätzler B, Dencher NA, Tittor J, Oesterhelt D, Yaniv-Checover S, Nachliel E, and Gutman M

Subjects

Arylsulfonates chemistry, Bacteriorhodopsins genetics, Cytoplasm metabolism, Energy Transfer, Extracellular Space metabolism, Halobacterium salinarum metabolism, Kinetics, Lasers, Motion, Mutagenesis, Site-Directed, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Bacteriorhodopsins chemistry, Bacteriorhodopsins metabolism, Protons, Purple Membrane chemistry, Purple Membrane metabolism

Abstract

The dynamics of proton transfer between the surface of purple membrane and the aqueous bulk have recently been investigated by the Laser Induced Proton Pulse Method. Following a Delta-function release of protons to the bulk, the system was seen to regain its state of equilibrium within a few hundreds of microseconds. These measurements set the time frame for the relaxation of any state of acid-base disequilibrium between the bacteriorhodopsin's surface and the bulk. It was also deduced that the released protons react with the various proton binding within less than 10 micro s. In the present study, we monitored the photocycle and the proton-cycle of photo-excited bacteriorhodopsin, in the absence of added buffer, and calculated the proton balance between the Schiff base and the bulk phase in a time-resolved mode. It was noticed that the late phase of the M decay (beyond 1 ms) is characterized by a slow (subsecond) relaxation of disequilibrium, where the Schiff base is already reprotonated but the pyranine still retains protons. Thus, it appears that the protonation of D96 is a slow rate-limiting process that generates a "proton hole" in the cytoplasmic section of the protein. The velocity of the hole propagation is modulated by the ionic strength of the solution and by selective replacements of charged residues on the interhelical loops of the protein, at domains that seems to be remote from the intraprotein proton conduction trajectory.

Published

2003

9. Stability of bacteriorhodopsin alpha-helices and loops analyzed by single-molecule force spectroscopy.

Author

Müller DJ, Kessler M, Oesterhelt F, Möller C, Oesterhelt D, and Gaub H

Subjects

Bacteriorhodopsins physiology, Bacteriorhodopsins ultrastructure, Elasticity, Hydrogen-Ion Concentration, Macromolecular Substances, Protein Conformation, Protein Denaturation, Protein Structure, Secondary, Protein Structure, Tertiary, Purple Membrane physiology, Purple Membrane ultrastructure, Stress, Mechanical, Bacteriorhodopsins chemistry, Microscopy, Atomic Force methods, Purple Membrane chemistry

Abstract

The combination of high-resolution atomic force microscopy imaging and single-molecule force spectroscopy allows the identification, selection, and mechanical investigation of individual proteins. In a recent paper we had used this technique to unfold and extract single bacteriorhodopsins (BRs) from native purple membrane patches. We show that subsets of the unfolding spectra can be classified and grouped to reveal detailed insight into the individualism of the unfolding pathways. We have further developed this technique and analysis to report here on the influence of pH effects and local mutations on the stability of individual structural elements of BR against mechanical unfolding. We found that, although the seven transmembrane alpha-helices predominantly unfold in pairs, each of the helices may also unfold individually and in some cases even only partially. Additionally, intermittent states in the unfolding process were found, which are associated with the stretching of the extracellular loops connecting the alpha-helices. This suggests that polypeptide loops potentially act as a barrier to unfolding and contribute significantly to the structural stability of BR. Chemical removal of the Schiff base, the covalent linkage of the photoactive retinal to the helix G, resulted in a predominantly two-step unfolding of this helix. It is concluded that the covalent linkage of the retinal to helix G stabilizes the structure of BR. Trapping mutant D96N in the M state of the proton pumping photocycle did not affect the unfolding barriers of BR.

Published

2002

10. Proton transfer dynamics on the surface of the late M state of bacteriorhodopsin.

Author

Nachliel E, Gutman M, Tittor J, and Oesterhelt D

Subjects

Biophysical Phenomena, Biophysics, Cell Membrane metabolism, Kinetics, Models, Molecular, Mutation, Protein Conformation, Time Factors, Bacteriorhodopsins metabolism, Cytoplasm metabolism, Protons

Abstract

The cytoplasmic surface of the BR (initial) state of bacteriorhodopsin is characterized by a cluster of three carboxylates that function as a proton-collecting antenna. Systematic replacement of most of the surface carboxylates indicated that the cluster is made of D104, E161, and E234 (Checover, S., Y. Marantz, E. Nachliel, M. Gutman, M. Pfeiffer, J. Tittor, D. Oesterhelt, and N. Dencher. 2001. Biochemistry. 40:4281-4292), yet the BR state is a resting configuration; thus, its proton-collecting antenna can only indicate the presence of its role in the photo-intermediates where the protein is re-protonated by protons coming from the cytoplasmic matrix. In the present study we used the D96N and the triple (D96G/F171C/F219L) mutant for monitoring the proton-collecting properties of the protein in its late M state. The protein was maintained in a steady M state by continuous illumination and subjected to reversible pulse protonation caused by repeated excitation of pyranine present in the reaction mixture. The re-protonation dynamics of the pyranine anion was subjected to kinetic analysis, and the rate constants of the reaction of free protons with the surface groups and the proton exchange reactions between them were calculated. The reconstruction of the experimental signal indicated that the late M state of bacteriorhodopsin exhibits an efficient mechanism of proton delivery to the unoccupied-most basic-residue on its cytoplasmic surface (D38), which exceeds that of the BR configuration of the protein. The kinetic analysis was carried out in conjunction with the published structure of the M state (Sass, H., G. Büldt, R. Gessenich, D. Hehn, D. Neff, R. Schlesinger, J. Berendzen, and P. Ormos. 2000. Nature. 406:649-653), the model that resolves most of the cytoplasmic surface. The combination of the kinetic analysis and the structural information led to identification of two proton-conducting tracks on the protein's surface that are funneling protons to D38. One track is made of the carboxylate moieties of residues D36 and E237, while the other is made of D102 and E232. In the late M state the carboxylates of both tracks are closer to D38 than in the BR (initial) state, accounting for a more efficient proton equilibration between the bulk and the protein's proton entrance channel. The triple mutant resembles in the kinetic properties of its proton conducting surface more the BR-M state than the initial state confirming structural similarities with the BR-M state and differences to the BR initial state.

Published

2002

11. Kinetics, energetics, and electronic coupling of the primary electron transfer reactions in mutated reaction centers of Blastochloris viridis.

Author

Huppman P, Arlt T, Penzkofer H, Schmidt S, Bibikova M, Dohse B, Oesterhelt D, Wachtveit J, and Zinth W

Subjects

Biophysical Phenomena, Biophysics, Electrochemistry, Electron Transport, Energy Metabolism, Kinetics, Models, Molecular, Photosynthesis, Photosynthetic Reaction Center Complex Proteins genetics, Point Mutation, Rhodopseudomonas genetics, Spectrophotometry, Thermodynamics, Alphaproteobacteria genetics, Alphaproteobacteria metabolism, Photosynthetic Reaction Center Complex Proteins chemistry, Photosynthetic Reaction Center Complex Proteins metabolism, Rhodopseudomonas metabolism

Abstract

Femtosecond spectroscopy in combination with site-directed mutagenesis has been used to study the dynamics of primary electron transfer in native and 12 mutated reaction centers of Blastochloris (B) (formerly called Rhodopseudomonas) viridis. The decay times of the first excited state P* vary at room temperature between of 0.6 and 50 ps, and at low temperatures between 0.25 and 90 ps. These changes in time constants are discussed within the scope of nonadiabatic electron transfer theory using different models: 1) If the mutation is assumed to predominantly influence the energetics of the primary electron transfer intermediates, the analysis of the room temperature data for the first electron transfer step to the intermediate P(+)B(A)(-) yields a reorganization energy lambda = 600 +/- 200 cm(-1) and a free energy gap Delta G ranging from -600 cm(-1) to 800 cm(-1). However, this analysis fails to describe the temperature dependence of the reaction rates. 2) A more realistic description of the temperature dependence of the primary electron transfer requires different values for the energetics and specific variations of the electronic coupling upon mutation. Apparently the mutations also lead to pronounced changes in the electronic coupling, which may even dominate the change in the reaction rate. One main message of the paper is that a simple relationship between mutation and a change in one reaction parameter cannot be given and that at the very least the electronic coupling is changed upon mutation.

Published

2002

12. Roles of cytoplasmic arginine and threonine in chloride transport by the bacteriorhodopsin mutant D85T.

Author

Paula S, Tittor J, and Oesterhelt D

Subjects

Anions, Bacteriorhodopsins chemistry, Biological Transport, Cell Line, Chlorine chemistry, Cytoplasm metabolism, Glutamine chemistry, Halorhodopsins, Kinetics, Light, Models, Biological, Models, Molecular, Mutagenesis, Mutagenesis, Site-Directed, Protein Binding, Protein Structure, Tertiary, Spectrophotometry, Valine chemistry, Arginine physiology, Bacteriorhodopsins genetics, Chlorine metabolism, Cytoplasm chemistry, Mutation, Threonine physiology

Abstract

In the light-driven anion pump halorhodopsin (HR), the residues arginine 200 and threonine 203 are involved in anion release at the cytoplasmic side of the membrane. Because of large sequence homology and great structural similarities between HR and bacteriorhodopsin (BR), it has been suggested that anion translocation by HR and by the chloride-pumping BR mutant BR-D85T occurs by the same mechanism. Consequently, the functions of the R200/T203 pair in HR should be the same as those of the corresponding pair in BR-D85T (R175/T178). We have put this hypothesis to a test by creating two mutants of BR-D85T in which R175 and T178 were replaced by glutamine and valine, respectively. Chloride transport activities were essentially the same for all three mutants, whereas chloride binding and the kinetics of parts of the photocycle were markedly affected by the replacement of T178. In contrast, the consequences of mutating R175 proved to be less significant. These findings are consistent with evidence obtained on HR and therefore support the idea that the respective mechanistic roles of the cytoplasmic arginine/threonine pairs in HR and BR-D85T are equal.

Published

2001

13. Conformations of the rhodopsin third cytoplasmic loop grafted onto bacteriorhodopsin.

Author

Heymann JB, Pfeiffer M, Hildebrandt V, Kaback HR, Fotiadis D, Groot B, Engel A, Oesterhelt D, and Müller DJ

Subjects

Amino Acid Sequence, Animals, Bacteriorhodopsins genetics, Bacteriorhodopsins ultrastructure, Cattle, Microscopy, Atomic Force, Models, Molecular, Molecular Sequence Data, Mutation, Protein Conformation, Protein Structure, Secondary, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins ultrastructure, Rhodopsin genetics, Rhodopsin ultrastructure, Bacteriorhodopsins chemistry, Rhodopsin chemistry

Abstract

Background: The third cytoplasmic loop of rhodopsin (Rho EF) is important in signal transduction from the retinal in rhodopsin to its G protein, transducin. This loop also interacts with rhodopsin kinase, which phosphorylates light-activated rhodopsin, and arrestin, which displaces transducin from light-activated phosphorylated rhodopsin., Results: We replaced eight residues of the EF loop of bacteriorhodopsin (BR) with 24 residues from the third cytoplasmic loop of bovine Rho EF. The surfaces of purple membrane containing the mutant BR (called IIIN) were imaged by atomic force microscopy (AFM) under physiological conditions to a resolution of 0.5-0.7 nm. The crystallinity and extracellular surface of IIIN were not perturbed, and the cytoplasmic surface of IIIN increased in height compared with BR, consistent with the larger loop. Ten residues of Rho EF were excised by V8 protease, revealing helices E and F in the AFM topographs. Rho EF was modeled onto the BR structure, and the envelope derived from the AFM data of IIIN was used to select probable models., Conclusions: A likely conformation of Rho EF involves some extension of helices E and F, with the tip of the loop lying over helix C and projecting towards the C terminus. This is consistent with mutagenesis data showing the TTQ transducin-binding motif close to loop CD, and cysteine cross-linking data indicating the C-terminal part of Rho EF to be close to the CD loop.

Published

2000

14. Unraveling photoexcited conformational changes of bacteriorhodopsin by time resolved electron paramagnetic resonance spectroscopy.

Author

Rink T, Pfeiffer M, Oesterhelt D, Gerwert K, and Steinhoff HJ

Subjects

Amino Acid Sequence, Amino Acid Substitution, Electron Spin Resonance Spectroscopy methods, Models, Molecular, Mutagenesis, Site-Directed, Photochemistry, Protein Conformation radiation effects, Protein Structure, Secondary, Recombinant Proteins chemistry, Recombinant Proteins radiation effects, Spin Labels, Time Factors, Bacteriorhodopsins chemistry, Bacteriorhodopsins radiation effects

Abstract

By means of time-resolved electron paramagnetic resonance (EPR) spectroscopy, the photoexcited structural changes of site-directed spin-labeled bacteriorhodopsin are studied. A complete set of cysteine mutants of the C-D loop, positions 100-107, and of the E-F loop, including the first alpha-helical turns of helices E and F, positions 154-171, was modified with a methanethiosulfonate spin label. The EPR spectral changes occurring during the photocycle are consistent with a small movement of helix C and an outward tilt of helix F. These helix movements are accompanied by a rearrangement of the E-F loop and of the C-terminal turn of helix E. The kinetic analysis of the transient EPR data and the absorbance changes in the visible spectrum reveals that the conformational change occurs during the lifetime of the M intermediate. Prominent rearrangements of nitroxide side chains in the vicinity of D96 may indicate the preparation of the reprotonation of the Schiff base. All structural changes reverse with the recovery of the bacteriorhodopsin initial state.

Published

2000

15. Azide reduces the hydrophobic barrier of the bacteriorhodopsin proton channel.

Author

Steinhoff HJ, Pfeiffer M, Rink T, Burlon O, Kurz M, Riesle J, Heuberger E, Gerwert K, and Oesterhelt D

Subjects

Azides pharmacology, Bacteriorhodopsins genetics, Bacteriorhodopsins radiation effects, Biophysical Phenomena, Biophysics, Cysteine chemistry, Electron Spin Resonance Spectroscopy, Hydrogen Bonding, Models, Molecular, Mutagenesis, Site-Directed, Nitrogen Oxides chemistry, Oxalates pharmacology, Protein Conformation, Protons, Spectroscopy, Fourier Transform Infrared, Spectrum Analysis, Raman, Spin Labels, Bacteriorhodopsins chemistry

Abstract

The sensitivity of a nitroxide spin label to the polarity of its environment has been used to estimate the hydrophobic barrier of the proton channel of the transmembrane proton pump bacteriorhodopsin. By means of site-specific mutagenesis, single cysteine residues were introduced at 10 positions located at the protein surface, in the protein interior, and along the proton pathway. After reaction with a methanethiosulfonate spin label, the principle values of the hyperfine tensor A and the g-tensor were determined from electron paramagnetic resonance spectra measured at 170 K. The shape of the hydrophobic barrier of the proton channel is characterized in terms of a polarity index, DeltaA, determined from the variation of the hyperfine coupling constant Azz. The maximum of the hydrophobic barrier is found to be close to the retinal chromophore in the proton uptake pathway. The effect of the asymmetric distribution of charged and polar residues in the proton release and uptake pathways is clearly reflected in the behavior of the hydrophobic barrier. The presence of azide reduces the barrier height of both the cytoplasmic and extracellular channels. This finding supports the view of azide and other weakly acidic anions as catalysts for the formation of hydrogen-bonded networks in proton pathways of proteins.

Published

1999

16. Evidence for charge-controlled conformational changes in the photocycle of bacteriorhodopsin.

Author

Sass HJ, Gessenich R, Koch MH, Oesterhelt D, Dencher NA, Büldt G, and Rapp G

Subjects

Bacteriorhodopsins genetics, Bacteriorhodopsins radiation effects, Biophysical Phenomena, Biophysics, Electrochemistry, Halobacterium salinarum chemistry, Halobacterium salinarum genetics, Halobacterium salinarum radiation effects, Hydrogen-Ion Concentration, Light, Mutagenesis, Site-Directed, Photochemistry, Protein Conformation, Spectrophotometry, Spectroscopy, Fourier Transform Infrared, X-Ray Diffraction, Bacteriorhodopsins chemistry

Abstract

The existence of two different M-state structures in the photocycle of the bacteriorhodopsin mutant ASP38ARG was proved. At pH 6.7 (0 to -6 degreesC) a spectroscopic M intermediate (M1) that does not differ significantly in its tertiary structure from the light-adapted ground state accumulates under illumination. At pH > 9 another state (M2), characterized by additional pronounced changes in the Fourier transform infrared difference spectrum in the region of the amide I and II bands, accumulates. The M2 intermediate trapped at pH 9.6 displays the same changes in the x-ray diffraction intensities under continuous illumination as previously described for x-ray experiments with the mutant ASP96ASN. These observations indicate that in this mutant the altered charge distribution at neutral pH controls the tertiary structural changes that seem to be necessary for proton translocation.

Published

1998

17. Low-temperature electron transfer from cytochrome to the special pair in Rhodopseudomonas viridis: role of the L162 residue.

Author

Ortega JM, Dohse B, Oesterhelt D, and Mathis P

Subjects

Amino Acid Sequence, Binding Sites, Cold Temperature, Electron Transport, Freezing, Heme metabolism, Kinetics, Models, Molecular, Oxidation-Reduction, Point Mutation, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Spectrophotometry, Thermodynamics, Tyrosine, Cytochrome c Group chemistry, Cytochrome c Group metabolism, Protein Conformation, Rhodopseudomonas metabolism

Abstract

Electron transfer from the tetraheme cytochrome c to the special pair of bacteriochlorophylls (P) has been studied by flash absorption spectroscopy in reaction centers isolated from seven strains of the photosynthetic purple bacterium Rhodopseudomonas viridis, where the residue L162, located between the proximal heme c-559 and P, is Y (wild type), F, W, G, M, T, or L. Measurements were performed between 294 K and 8 K, under redox conditions in which the two high-potential hemes of the cytochrome were chemically reduced. At room temperature, the kinetics of P+ reduction include two phases in all of the strains: a dominant very fast phase (VF), and a minor fast phase (F). The VF phase has the following t(1/2): 90 ns (M), 130 ns (W), 135 ns (F), 189 ns (Y; wild type), 200 ns (G), 390 ns (L), and 430 ns (T). These data show that electron transfer is fast whatever the nature of the amino acid at position L162. The amplitudes of both phases decrease suddenly around 200 K in Y, F, and W. The effect of temperature on the extent of fast phases is different in mutants G, M, L, and T, in which electron transfer from c-559 to P+ takes place at cryogenic temperatures in a substantial fraction of the reaction centers (T, 48%; G, 38%; L, 23%, at 40 K; and M, 28%, at 60 K), producing a stable charge separated state. In these nonaromatic mutants the rate of VF electron transfer from cytochrome to P+ is nearly temperature-independent between 294 K and 8 K, remaining very fast at very low temperatures (123 ns at 60 K for M; 251 ns at 40 K for L; 190 ns at 8 K for G, and 458 ns at 8 K for T). In all cases, a decrease in amplitudes of the fast phases is paralleled by an increase in very slow reduction of P+, presumably by back-reaction with Q(A)-. The significance of these results is discussed in relation to electron transfer theories and to freezing at low temperatures of cytochrome structural reorganization.

Published

1998

18. Localization of glycolipids in membranes by in vivo labeling and neutron diffraction.

Author

Weik M, Patzelt H, Zaccai G, and Oesterhelt D

Subjects

Amino Acids metabolism, Bacteriorhodopsins analysis, Fourier Analysis, Glucose analysis, Glycolipids chemistry, Mass Spectrometry, Molecular Weight, Neutrons, Protein Structure, Secondary, Sulfates analysis, Trisaccharides analysis, Trisaccharides metabolism, X-Ray Diffraction, Glycolipids analysis, Halobacterium salinarum chemistry, Purple Membrane chemistry

Abstract

Evidence is accumulating for the lateral organization of cell membrane lipids and proteins in the context of sorting or intracellular signaling. So far, however, information has been lacking on the details of protein-lipid interactions in such aggregates. Purple membranes are patches made up of lipids and the protein bacteriorhodopsin in the plasma membrane of certain Archaea. Naturally crystalline, they provide a unique opportunity to study the structure of a natural membrane at submolecular resolution by diffraction methods. We present a direct structural determination of the glycolipids with respect to bacteriorhodopsin in these membranes. Deuterium labels incorporated in vivo into the sugar moieties of the major glycolipid were localized by neutron diffraction. The data suggest a role for specific aromatic residue-carbohydrate stacking interactions in the formation of the purple membrane crystalline patches.

Published

1998

19. Spin-labeling studies of the conformational changes in the vicinity of D36, D38, T46, and E161 of bacteriorhodopsin during the photocycle.

Author

Rink T, Riesle J, Oesterhelt D, Gerwert K, and Steinhoff HJ

Subjects

Bacteriorhodopsins radiation effects, Electron Spin Resonance Spectroscopy, Halobacterium metabolism, Kinetics, Light, Models, Molecular, Mutagenesis, Site-Directed, Point Mutation, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Recombinant Proteins radiation effects, Spin Labels, Time Factors, Bacteriorhodopsins chemistry, Bacteriorhodopsins metabolism, Protein Conformation, Protein Structure, Secondary

Abstract

Electron paramagnetic resonance (EPR) spectroscopy of site-directed spin-labeled bacteriorhodopsin mutants is used to study structural changes during the photocycle. After exchange of the native amino acids D36 and D38 in the A-B loop, E161 in the E-F loop, and T46 in the putative proton channel by cysteines, these positions were modified by a methanethiosulfonate spin label. Time-resolved EPR spectroscopy reveals spectral changes during the photocycle for the mutants with spin labels attached to C36, C161, and C46. A comparison of the transient spectral amplitudes with simulated EPR difference spectra shows that the detected signals are due to changes in the spin label mobility and not to possible polarity changes in the vicinity of the attached spin label. The kinetic analysis of the EPR and the visible data with a global fitting procedure exhibits a structural rearrangement near position 161 in the E-F loop in the M state. The environmental changes at positions 36 and 46, however, occur during the M-to-N transition. All structural changes reverse with the recovery of the BR ground state. No structural changes are detected with a spin label attached to C38.

Published

1997

20. pH-induced structural changes in bacteriorhodopsin studied by Fourier transform infrared spectroscopy.

Author

Száraz S, Oesterhelt D, and Ormos P

Subjects

Aspartic Acid, Bacteriorhodopsins isolation & purification, Bacteriorhodopsins metabolism, Carbon Isotopes, Halobacterium salinarum metabolism, Hydrogen-Ion Concentration, Kinetics, Magnetic Resonance Spectroscopy, Point Mutation, Protein Conformation, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Spectroscopy, Fourier Transform Infrared instrumentation, Spectroscopy, Fourier Transform Infrared methods, Structure-Activity Relationship, Bacteriorhodopsins chemistry

Abstract

Previous C13-NMR studies showed that two of the four internal aspartic acid residues (Asp-96 and Asp-115) of bacteriorhodopsin (bR) are protonated up to pH = 10, but no accurate pKa of these residues has been determined. In this work, infrared spectroscopy with the attenuated total reflection technique was used to characterize pH-dependent structural changes of ground-state, dark-adapted wild-type bacteriorhodopsin and its mutant (D96N) with aspartic acid-96 replaced by asparagine. Data indicated deprotonation of Asp-96 at high pH (pKa = 11.4 +/- 0.1), but no Asp-115 titration was observed. The analysis of the whole spectral region characteristic to complex conformational changes in the protein showed a more complicated titration with an additional pKa value (pKa1 = 9.3 +/- 0.3 and pKa2 = 11.5 +/- 0.2). Comparison of results obtained for bR and the D96N mutant of bR shows that the pKa approximately 11.5 characterizes not a direct titration of Asp-96 but a protein conformational change that makes Asp-96 accessible to the external medium.

Published

1994

21. Inversion of proton translocation in bacteriorhodopsin mutants D85N, D85T, and D85,96N.

Author

Tittor J, Schweiger U, Oesterhelt D, and Bamberg E

Subjects

Cloning, Molecular, Darkness, Electrochemistry methods, Escherichia coli, Genetic Vectors, Halobacterium metabolism, Hydrogen-Ion Concentration, Kinetics, Light, Mutagenesis, Photolysis, Polymerase Chain Reaction, Retinaldehyde analogs & derivatives, Retinaldehyde metabolism, Schiff Bases, Spectrophotometry, Bacteriorhodopsins chemistry, Bacteriorhodopsins metabolism, Point Mutation

Abstract

Proton translocation activity of bacteriorhodopsin mutants lacking the proton acceptor Asp-85 was investigated using the black lipid membrane technique. Mutants D85N, D85T, and D85,96N were constructed and homologously expressed in Halobacterium salinarium to yield a membrane fraction with a buoyant density of 1.18 g/cm3, i.e., identical to that of wild-type purple membrane. In all mutants, the absorbance maximum was red-shifted between 27 and 49 nm compared with wild type, and the pKa values of the respective Schiff bases were reduced to between 8.3 and 8.9 compared with the value of > 13 in wild type. Therefore, a mixture of chromophores absorbing at 410 nm (deprotonated form) and around 600 nm (protonated form) exists at physiological pH. In continuous blue light, the deprotonated form generates stationary photocurrents. The currents are enhanced by a factor of up to 50 upon addition of azide in D85N and D85,96N mutants, whereas D85T shows no azide effect. The direction of these currents is the same as in wild type in yellow light. Yellow light alone is not sufficient to generate stationary currents in the mutants, but increasing yellow light intensity in the presence of blue light leads to an inversion of the current. Because all currents are carried by protons, this two-photon process demonstrates an inverted proton translocation by BR mutants.

Published

1994

22. Photochemical conversion of the O-intermediate to 9-cis-retinal-containing products in bacteriorhodopsin films.

Author

Popp A, Wolperdinger M, Hampp N, Brüchle C, and Oesterhelt D

Subjects

Biophysical Phenomena, Biophysics, Diterpenes, Halobacterium salinarum chemistry, Halobacterium salinarum radiation effects, Holography, Isomerism, Models, Chemical, Photochemistry, Retinaldehyde chemistry, Retinaldehyde radiation effects, Spectrophotometry, Bacteriorhodopsins chemistry, Bacteriorhodopsins radiation effects

Abstract

The photochemical activity of the O-state was investigated in bacteriorhodopsin (BR) films containing wildtype BR at pH 6.5 in the presence of glycerol. The formation of a photoproduct of O with an absorption maximum at 490 nm and 9-cis-retinal configuration was found. This 490-nm product was named P and shows a slow thermal reaction into a compound with a maximal absorption at 380 nm which was named Q and contains free 9-cis-retinal in the proteins binding site. The photoproducts of O, i.e., P and Q, are very similar, or even identical, to those previously observed in blue membranes. Common to the O-state and blue membrane forms of bacteriorhodopsin is a protonated aspartic acid 85, and we suggest that it is the reduced negative charge around the Schiff base which is responsible for the 9-cis photoisomerization. The release of a proton from aspartic acid 85 is linked to the conversion of the O-state back to the initial state of BR. Therefore the conditions of low proton mobility in BR films containing glycerol favor the accumulation of the O-state. For optical and holographic applications such BR films are very attractive. It is possible to create photoproducts with red light which are thermally stable at room temperature and that can be photochemically erased. Dependent on the light composition both properties can be realized in the same sample material. This feature may bridge the gap between information processing and short-term and long-term storage of information with BR.

Published

1993

23. Bacteriorhodopsin wildtype and variant aspartate-96 --> aspargine as reversible holographic media.

Author

Hampp N, Bräuchle C, and Oesterhelt D

Abstract

Air dried films of purple membranes (PM) from Halobacterium halobium containing the photochromic protein bacteriorhodopsin (BR) were prepared and the BR-photocycle of this material analyzed. The absorption maxima of the initial state B (lambda(max) = 570 nm) and the photochemical intermediate M (lambda(max) = 412 nm), which is the longest living intermediate in suspension (tau approximately 10 ms), were spectrally well separated. Light-induced population gratings between B and M were used for reversible holographic recording in these dry PM films. The resolution (>5,000 lines/mm) of PM films was comparable to the corresponding values of conventional photochromic recording materials. The longterm stability toward photochemical degradation of PM films is excellent (> 100.000 recording cycles). The spectral bandwidth (400-680 nm) of such films covers nearly the whole visible spectrum. Both the photochemical transition from B --> M with wavelengths in the green-red range and from M --> B with blue light were utilized for holographic recording. The latter possibility (M --> B) seems to be advantageous for several applications because the holographic grating is only formed during reconstruction. Higher reading intensities lead to higher population of the M-state and result in an increase of the fringe contrast instead of decreasing it. New possibilities for the further development of holographic media based on bacteriorhodopsin are raised by the availability of PM variants with modified optical properties. By the use of the variant BR-326, which differs from the wildtype PM by a single amino acid exchange (aspartate-96 --> asparagine), the sensitivity of PM films is increased by approximately 50% from 12 cm(2)/J to 19 cm(2)/J for recording with 568 nm. The sensitivity for recording with 413 nm (33 cm(2)/J) is not influenced by the amino acid exchange. The observed diffraction efficiency eta of PM films with BR-326 is twice that of BR-wildtype (BR-WT) films and is in the range of conventional organic photochromics ( approximately 1%). In dried films of both BR-WT and BR-326 the M-decay was shown to be at least biexponential.

Published

1990

24. Photolysis of bacterial rhodopsin.

Author

Chu Kung M, DeVault D, Hess B, and Oesterhelt D

Subjects

Kinetics, Lasers, Photolysis, Spectrophotometry, Bacteriorhodopsins, Carotenoids, Halobacterium

Published

1975

25. Picosecond events in the photochemical cycle of the light-driven chloride-pump halorhodopsin.

Author

Polland HJ, Franz MA, Zinth W, Kaiser W, Hegemann P, and Oesterhelt D

Subjects

Chlorides, Halorhodopsins, Models, Chemical, Photochemistry, Spectrometry, Fluorescence, Time Factors, Bacteriorhodopsins, Carotenoids

Abstract

The early events in halorhodopsin after light excitation are studied with picosecond time resolution. Absorption and fluorescence measurements show that the electronically excited state of the incorporated retinal has a lifetime of 5 ps. Within that time a red-shifted photoproduct is formed that remains stable for at least 2 ns.

Published

1985

26. Early picosecond events in the photocycle of bacteriorhodopsin.

Author

Polland HJ, Franz MA, Zinth W, Kaiser W, Kölling E, and Oesterhelt D

Abstract

The primary processes of the photochemical cycle of light-adapted bacteriorhodopsin (BR) were studied by various experimental techniques with a time resolution of 5 x 10(-13) s. The following results were obtained. (a) After optical excitation the first excited singlet state S(1) of bacteriorhodopsin is observed via its fluorescence and absorption properties. The population of the excited singlet state decays with a lifetime tau(1) of approximately 0.7 ps (430 +/- 50 fs) (52). (b) With the same time constant the first ground-state intermediate J builds up. Its absorption spectrum is red-shifted relative to the spectrum of BR by approximately 30 nm. (c) The second photoproduct K, which appears with a time constant of tau(2) = 5 ps shows a red-shift of 20 nm, relative to the peak of BR. Its absorption remains constant for the observation time of 300 ps. (d) Upon suspending bacteriorhodopsin in D(2)O and deuterating the retinal Schiff base at its nitrogen (lysine 216), the same photoproducts J and K are observed. The relaxation time constants tau(1) and tau(2) remain unchanged upon deuteration within the experimental accuracy of 20%.

Published

1986

27. The photochemical cycle of halorhodopsin: absolute spectra of intermediates obtained by flash photolysis and fast difference spectra measurements.

Author

Tittor J, Oesterhelt D, Maurer R, Desel H, and Uhl R

Abstract

Results of experiments using flash photolysis and fast difference spectroscopy suggest an extended version of the earlier published scheme of the photochemical cycle of halorhodopsin. Detailed experimental verification of the suggested photocycle is given. Due to the high resolution of the time-resolved difference spectra, absolute spectra of the intermediates in the photocycle were derived, allowing the interpretation of complex kinetic absorbance changes.

Published

1987

28. Low temperature kinetics of H+ changes of bacterial rhodopsin.

Author

Chance B, Porte M, Hess B, and Oesterhelt D

Subjects

Kinetics, Photolysis, Temperature, Bacteriorhodopsins, Carotenoids, Hydrogen-Ion Concentration

Published

1975

29. Chromophore equilibria in bacteriorhodopsin.

Author

Fischer U and Oesterhelt D

Subjects

Anions, Kinetics, Lysine, Photochemistry, Retinaldehyde analysis, Spectrophotometry instrumentation, Spectrophotometry methods, Bacteriorhodopsins, Carotenoids

Abstract

An investigation of the dark equilibria between different chromophores of bacteriorhodopsin (BR) and studies of the kinetics of their interconversion and photochemical activity have led to the following conclusions. (a) A component of the 605-nm chromophore of BR decays in the millisecond range and is likely to be identical to the intermediate O of the photochemical cycle of BR and is assumed to be formed from the purple complex (PC) by the binding of one proton to BR. (b) An acidic form the PC, PCaL-, arises from the 605-nm chromophore by selective binding of anions L- (F- greater than Cl- greater than Br- greater than I- greater than Cl04-) to BR. (c) The isomeric equilibrium between 13-cis and all-trans retinal is approximately 0.15/0.85 in PCaCl-, 0.3/0.7 in the 605-nm chromophore as compared to 0.5/0.5 in the PC. (d) The 500-nm chromophore is formed from the PC by release of nearly one proton from BR. (e) The pH range in which the PC exists is reduced in a high-temperature structure of the purple membrane as compared to its low temperature structure. A model for the chromophore structure is proposed as a hypothesis, which allows a comprehensive interpretation of the results. In this model the absorption spectrum of the retinylidene lysine Schiff base is modulated by its protonation state and the interaction with an anionic group.

Published

1979

30. Changes in the protonation state of bacterio-opsin during reconstitution of bacteriorhodopsin.

Author

Fischer UC and Oesterhelt D

Subjects

Apoproteins, Chemical Phenomena, Chemistry, Diterpenes, Halobacterium, Hydrogen-Ion Concentration, Isomerism, Light, Models, Chemical, Protons, Ultraviolet Rays, Bacteriorhodopsins radiation effects, Carotenoids radiation effects, Retinaldehyde radiation effects, Vitamin A analogs & derivatives

Abstract

Protonation changes of the protein occur during the reconstitution of bacteriorhodopsin from bacterio-opsin and all-trans retinal in the purple membrane of Halobacterium halobium. The protonation changes are conveniently determined from measures of the pH changes after photoisomerisation of 9-cis retinal in apomembrane preparations, which induces the reconstitution. In addition, to the omega-amino group of the lysine which is involved in the condensation of retinal and bacterio-opsin, the dissociation equilibria of at least two other amino acid residues are changed during the reconstitution. The results are consistent with a proposed model of chromophore structure in which an interaction of the Schiff's base occurs with two protonable amino acid residues.

Published

1980

31. The effect of protonation and electrical interactions on the stereochemistry of retinal schiff bases.

Author

Tavan P, Schulten K, and Oesterhelt D

Abstract

Based on quantumchemical MNDOC calculations it is shown that the ground-state properties of a retinal Schiff base depend sensitively on its protonation state and charge environment. This is exemplified for the equilibrium geometry, for the distribution of partial charges and, in particular, for the thermal isomerization barriers around the pi-bonds. It is demonstrated that a protein, by protonating the retinal Schiff base and by providing one or two negative ions in its environment, can reduce double-bond isomerization barriers from 50 kcal/mol for the unprotonated compound to approximately 5 kcal/mol and can increase single bond barriers from 5 kcal/mol to approximately 20 kcal/mol. Thereby, the specific location of the ions relative to the polyene chain of the protonated retinal Schiff base determines the barrier heights. The results explain the ground-state isomerization reactions of retinal observed in bacteriorhodopsin and in squid retinochrome.

Published

1985

32. Substituents at the c(13) position of retinal and their influence on the function of bacteriorhodopsin.

Author

Tavan P, Schulten K, Gärtner W, and Oesterhelt D

Abstract

Retinal analogues in which the 13-methyl group is replaced by H, C(2)H(5), CF(3), and OCH(3) residues are studied by means of quantumchemical modified neglect of diatomic overlap-correlated version (MNDOC) calculations. The analogues are suitable to test the stereochemical mechanism of proton pumping in bacteriorhodopsin. The results explain the proton-pumping activities of bacterio-opsin reconstituted with these analogues and elucidate the decisive role of retinal's ground-state intramolecular properties in the pump cycle of bacteriorhodopsin.

Published

1985